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A high frequency of sequence alterations is due to formalin fixation of archival specimens.较高频率的序列改变是由于存档标本的福尔马林固定所致。
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2
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本文引用的文献

1
p53 Mutations in lung cancer associated with residential radon exposure.与居住环境中氡暴露相关的肺癌中的p53突变。
Cancer Epidemiol Biomarkers Prev. 1999 May;8(5):433-8.
2
Clones of normal keratinocytes and a variety of simultaneously present epidermal neoplastic lesions contain a multitude of p53 gene mutations in a xeroderma pigmentosum patient.在一名着色性干皮病患者中,正常角质形成细胞的克隆以及多种同时存在的表皮肿瘤性病变含有大量p53基因突变。
Cancer Res. 1998 Jun 1;58(11):2449-55.
3
Genomic analysis of single cells from human basal cell cancer using laser-assisted capture microscopy.使用激光辅助捕获显微镜对人基底细胞癌的单细胞进行基因组分析。
Mutat Res. 1997 Sep;382(1-2):45-55. doi: 10.1016/s1383-5726(97)00008-3.
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Molecular pathology in basal cell cancer with p53 as a genetic marker.以p53作为基因标志物的基底细胞癌中的分子病理学
Oncogene. 1997 Aug 28;15(9):1059-67. doi: 10.1038/sj.onc.1201435.
5
Benign clonal keratinocyte patches with p53 mutations show no genetic link to synchronous squamous cell precancer or cancer in human skin.具有p53突变的良性克隆性角质形成细胞斑块与人类皮肤中的同步鳞状细胞癌前病变或癌症无遗传关联。
Am J Pathol. 1997 May;150(5):1791-803.
6
The role of DNase and EDTA on DNA degradation in formaldehyde fixed tissues.脱氧核糖核酸酶(DNase)和乙二胺四乙酸(EDTA)在甲醛固定组织中对DNA降解的作用。
Biotech Histochem. 1996 May;71(3):123-9. doi: 10.3109/10520299609117148.
7
Human epidermal cancer and accompanying precursors have identical p53 mutations different from p53 mutations in adjacent areas of clonally expanded non-neoplastic keratinocytes.人类表皮癌及其伴随的癌前病变具有相同的p53突变,这些突变不同于克隆性扩增的非肿瘤性角质形成细胞相邻区域中的p53突变。
Oncogene. 1996 Feb 15;12(4):765-73.
8
Direct solid-phase sequence analysis of the human p53 gene by use of multiplex polymerase chain reaction and alpha-thiotriphosphate nucleotides.利用多重聚合酶链反应和α-硫代三磷酸核苷酸对人p53基因进行直接固相序列分析。
Clin Chem. 1995 Oct;41(10):1461-6.
9
Fidelity of DNA synthesis by the Thermus aquaticus DNA polymerase.嗜热水生栖热菌DNA聚合酶的DNA合成保真度
Biochemistry. 1988 Aug 9;27(16):6008-13. doi: 10.1021/bi00416a027.
10
Direct solid phase sequencing of genomic and plasmid DNA using magnetic beads as solid support.以磁珠作为固相支持物对基因组DNA和质粒DNA进行直接固相测序。
Nucleic Acids Res. 1989 Jul 11;17(13):4937-46. doi: 10.1093/nar/17.13.4937.

较高频率的序列改变是由于存档标本的福尔马林固定所致。

A high frequency of sequence alterations is due to formalin fixation of archival specimens.

作者信息

Williams C, Pontén F, Moberg C, Söderkvist P, Uhlén M, Pontén J, Sitbon G, Lundeberg J

机构信息

Department of Biotechnology, KTH Royal Institute of Technology, Stockholm University Hospital, Sweden.

出版信息

Am J Pathol. 1999 Nov;155(5):1467-71. doi: 10.1016/S0002-9440(10)65461-2.

DOI:10.1016/S0002-9440(10)65461-2
PMID:10550302
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1866966/
Abstract

Genomic analysis of archival tissues fixed in formalin is of fundamental importance in biomedical research, and numerous studies have used such material. Although the possibility of polymerase chain reaction (PCR)-introduced artifacts is known, the use of direct sequencing has been thought to overcome such problems. Here we report the results from a controlled study, performed in parallel on frozen and formalin-fixed material, where a high frequency of nonreproducible sequence alterations was detected with the use of formalin-fixed tissues. Defined numbers of well-characterized tumor cells were amplified and analyzed by direct DNA sequencing. No nonreproducible sequence alterations were found in frozen tissues. In formalin-fixed material up to one mutation artifact per 500 bases was recorded. The chance of such artificial mutations in formalin-fixed material was inversely correlated with the number of cells used in the PCR-the fewer cells, the more artifacts. A total of 28 artificial mutations were recorded, of which 27 were C-T or G-A transitions. Through confirmational sequencing of independent amplification products artifacts can be distinguished from true mutations. However, because this problem was not acknowledged earlier, the presence of artifacts may have profoundly influenced previously reported mutations in formalin-fixed material, including those inserted into mutation databases.

摘要

对用福尔马林固定的存档组织进行基因组分析在生物医学研究中至关重要,并且已有大量研究使用了此类材料。尽管已知存在聚合酶链反应(PCR)引入的假象的可能性,但人们认为直接测序的使用可以克服此类问题。在此,我们报告一项对照研究的结果,该研究对冷冻材料和福尔马林固定材料同时进行,结果发现使用福尔马林固定组织时检测到了高频的不可重复序列改变。通过直接DNA测序对确定数量的特征明确的肿瘤细胞进行扩增和分析。在冷冻组织中未发现不可重复的序列改变。在福尔马林固定材料中,每500个碱基记录到多达一个突变假象。福尔马林固定材料中出现此类人工突变的几率与PCR中使用的细胞数量呈负相关——细胞数量越少,假象越多。总共记录到28个人工突变,其中27个是C-T或G-A转换。通过对独立扩增产物进行验证性测序,可以将假象与真实突变区分开来。然而,由于这个问题之前未被认识到,假象的存在可能对先前报道的福尔马林固定材料中的突变产生了深远影响,包括那些录入突变数据库中的突变。